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一种微丝相关信号转导颗粒中含p185(neu)的糖蛋白复合物。纯化、重组以及与p58(gag)和肌动蛋白的分子关联。

The p185(neu)-containing glycoprotein complex of a microfilament-associated signal transduction particle. Purification, reconstitution, and molecular associations with p58(gag) and actin.

作者信息

Li Y, Hua F, Carraway K L, Carraway C A

机构信息

Department of Biochemistry and Molecular Biology, University of Miami School of Medicine, Miami, Florida 33101, USA.

出版信息

J Biol Chem. 1999 Sep 3;274(36):25651-8. doi: 10.1074/jbc.274.36.25651.

Abstract

Microfilaments associate with the microvillar membrane of 13762 ascites mammary adenocarcinoma cells via a large transmembrane complex (TMC) comprising the major glycoproteins TMC-gp120, -110, -80, -65, and -55, the receptor kinase p185(neu), and the cytoplasmic proteins actin and p58(gag), linking the receptor with microfilaments in a signal transduction particle. Immunoblot screening with polyclonal antisera to TMC glycoproteins showed selective epithelial expression in normal rat tissues and epithelially derived tumor cells. The TMC glycoproteins were isolated by solubilization of microfilament core preparations in SDS, dilution, and separation on a concanavalin A-agarose affinity column. The large p185(neu)-containing complex was reconstituted from the column eluate after displacement of SDS with nonionic detergent, demonstrated by gel filtration and co-immunoprecipitation of the glycoproteins with anti-gp55 or anti-p185(neu). Exhaustive biotinylation of the glycoproteins gave a stoichiometry of gp120:gp110:gp80:gp65:gp55 of approximately 1:1:1:0.5:1. Overlay blots with biotinylated actin and in vitro translated, [(35)S]methionine-labeled p58(gag), respectively, showed specific interactions of actin with gp55 and gp120 and of p58(gag) with gp65 and gp55. These results provide evidence for a specific complex of microfilament-associated glycoproteins containing p185(neu) and p58(gag) and suggest a role for the complex in signal transduction scaffolding.

摘要

微丝通过一个大型跨膜复合物(TMC)与13762腹水型乳腺腺癌细胞的微绒毛膜相连,该复合物包含主要糖蛋白TMC-gp120、-110、-80、-65和-55、受体激酶p185(neu)以及细胞质蛋白肌动蛋白和p58(gag),在一个信号转导颗粒中将受体与微丝连接起来。用针对TMC糖蛋白的多克隆抗血清进行免疫印迹筛选显示,在正常大鼠组织和上皮来源的肿瘤细胞中存在选择性上皮表达。通过在SDS中溶解微丝核心制剂、稀释并在伴刀豆球蛋白A-琼脂糖亲和柱上分离,可分离出TMC糖蛋白。在用非离子去污剂取代SDS后,从柱洗脱物中重构了含大的p185(neu)的复合物,通过凝胶过滤以及糖蛋白与抗gp55或抗p185(neu)的共免疫沉淀得以证明。对糖蛋白进行彻底的生物素化后,得到的gp120:gp110:gp80:gp65:gp55化学计量比约为1:1:1:0.5:1。分别用生物素化的肌动蛋白和体外翻译的、[³⁵S]甲硫氨酸标记的p58(gag)进行覆盖印迹,结果显示肌动蛋白与gp55和gp120以及p58(gag)与gp65和gp55之间存在特异性相互作用。这些结果为含有p185(neu)和p58(gag)的微丝相关糖蛋白的特异性复合物提供了证据,并表明该复合物在信号转导支架中发挥作用。

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